Activator protein transcription factors coordinate human IL-33 expression from noncanonical promoters in chronic airway disease
Heather E. Raphael, Ghandi F. Hassan, Omar A. Osorio, Lucy S. Cohen, Morgan D. Payne, Ella Katz-Kiriakos, Ishana Tata, Jamie Hicks, Derek E. Byers, Bo Zhang, Jen Alexander-Brett
Heather E. Raphael, Ghandi F. Hassan, Omar A. Osorio, Lucy S. Cohen, Morgan D. Payne, Ella Katz-Kiriakos, Ishana Tata, Jamie Hicks, Derek E. Byers, Bo Zhang, Jen Alexander-Brett
View: Text | PDF
Research Article Immunology Pulmonology

Activator protein transcription factors coordinate human IL-33 expression from noncanonical promoters in chronic airway disease

Abstract

IL-33 is a cytokine central to type 2 immune pathology in chronic airway disease. This cytokine is abundantly expressed in the respiratory epithelium and increased in disease, but how expression is regulated is undefined. Here we show that increased IL33 expression occurs from multiple noncanonical promoters in human chronic obstructive pulmonary disease (COPD), and it facilitates production of alternatively spliced isoforms in airway cells. We found that phorbol 12-myristate 13-acetate (PMA) can activate IL33 promoters through protein kinase C in primary airway cells and lines. Transcription factor (TF) binding arrays combined with RNA interference identified activator protein (AP) TFs as regulators of baseline and induced IL33 promoter activity. ATAC-Seq and ChIP-PCR identified chromatin accessibility and differential TF binding as additional control points for transcription from noncanonical promoters. In support of a role for these TFs in COPD pathogenesis, we found that AP-2 (TFAP2A, TFAP2C) and AP-1 (FOS and JUN) family members are upregulated in human COPD specimens. This study implicates integrative and pioneer TFs in regulating IL33 promoters and alternative splicing in human airway basal cells. Our work reveals a potentially novel approach for targeting IL-33 in development of therapeutics for COPD.

Authors

Heather E. Raphael, Ghandi F. Hassan, Omar A. Osorio, Lucy S. Cohen, Morgan D. Payne, Ella Katz-Kiriakos, Ishana Tata, Jamie Hicks, Derek E. Byers, Bo Zhang, Jen Alexander-Brett

×

Figure 2

IL33 spliced isoform is derived from a noncanonical promoter.

Options: View larger image (or click on image) Download as PowerPoint
IL33 spliced isoform is derived from a noncanonical promoter. (A) Trans...
(A) Transcript mRNA levels measured in cultured airway basal cells using promoter-specific qPCR assays as in Figure 1, quantified from n = 12 non-COPD and n = 25 COPD specimens. (B) Nested PCR based on isoform-specific cDNA generation followed by amplification using primers encompassing the IL33 coding region. Primer sets are color coded according to location, and assay steps are as depicted in the schematic. Agarose gel analysis for a subset of COPD specimens demonstrating truncated bands observed only for PCR amplification on IL33B. (C) qPCR using primer-probe sets designed to detect the truncated IL33Δ34 transcript using random primer-generated cDNA template from A, quantified as copy/mL using plasmid standard and normalized to GAPDH. Statistical analysis included t test (A and C). Data in A are representative of n = 2 technical replicates; experiments in B and C were repeated in triplicate.